Ronchi A, Nicolis S, Santoro C, Ottolenghi S
Dipartimento di Genetica e di Biologia dei Microrganismi, Università di Milano, Italy.
Nucleic Acids Res. 1989 Dec 25;17(24):10231-41. doi: 10.1093/nar/17.24.10231.
The -198 T----C mutation in the promoter of the A gamma-globin gene increases 20-30 fold the expression of this gene in adult erythroid cells of patients (Hereditary Persistence of Fetal Hemoglobin, HPFH). We show here that this mutation creates a strong binding site, resembling a CACCC box, for two ubiquitous nuclear proteins, one of which is Sp1. The mutated promoter is four to five-fold more efficient than a normal gamma-globin promoter in driving expression of a CAT reporter plasmid when transfected into erythroid cells. The overexpression of the mutant is abolished by the introduction of an additional mutation disrupting the new binding site. No overexpression of the mutant is observed in non-erythroid cells, indicating that the ubiquitous factors bound on the mutated sequence must cooperate with erythroid specific factors.
γ-珠蛋白基因启动子中的-198 T----C突变使该基因在患者(遗传性胎儿血红蛋白持续存在,HPFH)的成年红细胞中的表达增加20至30倍。我们在此表明,该突变产生了一个类似于CACCC盒的强结合位点,可与两种普遍存在的核蛋白结合,其中一种是Sp1。当转染到红细胞中时,突变型启动子在驱动CAT报告质粒表达方面比正常γ-珠蛋白启动子效率高4至5倍。通过引入破坏新结合位点的额外突变,突变体的过表达被消除。在非红细胞中未观察到突变体的过表达,这表明结合在突变序列上的普遍存在的因子必须与红细胞特异性因子协同作用。
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